Journal of Clinical Chemistry and Clinical Biochemistry Zeitschrift für Klinische Chemie und

Summary: We describe an interesting and novel alternative to conventional irrtmunoassay techniques for the measure­ment of antigens and antibodies in body fluids. The label used for all assays is a pyruvate kinase-IgG conjugate of the relevant second (species-specific) antibody. All assays follow the same principle in which a solid phase antigen is used to adsorb unreacted first (substance-specific) antibody following a conventional antibody-antigen reaction in a liquid phase. After washing, the solid phase antigen-first antibody is allowed to react with the labelled second antibody. The solid phase is then washed and the pyruvate kinase bound to the solid phase is used to generate ATP which is measured kinetically in a luminometer. Assays are described for insulin, insulin antibodies and gentamicin to demonstrate both the versatility and sensitivity of this type of assay. The insulin assay had a lower detection limit of under 0.25 /iU per tube and was comparable with the radioimmuno­assay used for routine purposes both in sensitivity and reproducibility. The insulin antibody assay correlated well with the radiometric determination used routinely in the laboratory. The gentamicin assay correlated well with the routine commercial radioimmunoassay and also had comparable co­efficients of variation. In all cases, the inter- and intra-assay variation was under 10% in the range of interest.